Infect Immun. TNF- to human being or murine macrophages infected with resulted in improved intracellular killing of mycobacteria (4, 10, 19). Similarly, treatment of infected mice with TNF-, with or without interleukin 2 (IL-2), resulted in a decrease in the mycobacterial burden in the spleens and livers of the animals (6, 8). In another study, however, an additive decrease in resistance as measured by an increase in mycobacterial CFU was observed in mice treated with a combination of antibodies to TNF- and gamma interferon (IFN-) compared to that observed after administration of either antibody only (1). The addition of pentoxifylline, a chemical inhibitor of TNF-, to mice show impaired phagocytic (13), NK (3, 29, 30), and T (2, 33)-cell functions, which constitute important mechanisms of immunoregulation and sources of TNF-. The current study also evaluated the energy of C57BL/6 mice (5 to 6 weeks older) were used in experiments which compared disease progression and serum TNF- production among the different strains of mice. All animals (Jackson Laboratories, Pub Harbor, Maine) were randomized and housed in groups of no more than five in microisolator cages and were fed ad libitum. Illness of mice. Mac pc strain 101 (Mac pc 101) was cultured on Middlebrook 7H11 agar plates (Remel, Lenexa, Kan.). After 2 to 3 3 weeks of incubation, transparent colonies of Mac pc 101 were picked from your plates, suspended in sterile Middlebrook 7H9 broth (Difco Laboratories, Detroit, Mich.), aliquoted, and freezing at ?70C as the stock culture (5 108 to 1 1 109 CFU/ml) for those infection studies. The mice were infected intravenously with 5 to 6 107 CFU of Mac pc 101 in 7H9 broth. Control mice were sham infected with broth. Groups of five animals were sacrificed at weeks 1, 3, 5, and 8 following infection and evaluated for body weight, organ excess weight (spleen, liver, and lung), and microbial burden in the weighed subsections of these organs. Blood was collected for measurement of TNF- levels in the serum. A separate group of each strain of mice, infected (= 20) and uninfected (= 10), was set aside for any survival study. Microbial burden. Weighed sections of cells (liver, lung, and spleen) were homogenized in Middlebrook 7H9 medium (Difco), and aliquots from different dilutions were plated onto Middlebrook 7H11 agar plates (Remel) in triplicate. The ethnicities were incubated for 3 weeks at 37C in 7% CO2. TNF- levels. TNF- levels in the sera were measured by an enzyme-linked immunosorbent assay with kits from Genzyme Diagnostics (Cambridge, Mass.). Treatment with TNF- inhibitors and measurement of disease progression. C57BL/6 value was found to be less than 0.05; consequently, no adjustment was imposed within the pairwise assessment of values. Variations in various guidelines (including body weight, organ excess weight, microbial burden, and serum TNF- level) were determined by analysis of variance. Results of the microbial burden (in CFU) were analyzed after log transformation of the data. All ideals reported are the results of two-tailed assessments, with no adjustment for multiple comparisons. RESULTS Susceptibility of C57BL/6 (and +/+ mice (week 5). However, by week 6, the mortality rates for mice. Mortality in mice continued to increase throughout the observation period, whereas the mortality rates stabilized at week 8 for both 0.05). The pairwise comparison showed the susceptibility of the strain (= 0.144). The +/+ mice were the least susceptible and were statistically different from the strain of mice (= 0.014) but not from your = 0.373). Mycobacterial disease progression, as measured by increased organ weights (splenomegaly or hepatomegaly) and microbial burden, also developed in C57BL/6 mice at most time points. TABLE 1 Relative organ weights in three strains of C57BL/6 mice at 3 weeks following infection with MAC?101 0.05 compared to uninfected control.? Open in a separate windows FIG. 2 Microbial burden in three strains.II. cultures or animals infected with a sp. has been associated with increased resistance to the infection, and inhibition of TNF- has been reported to decrease resistance. In vitro addition of TNF- to human or murine macrophages infected with resulted in increased intracellular killing of mycobacteria (4, 10, 19). Similarly, treatment of infected mice with TNF-, with or without interleukin 2 (IL-2), resulted in a decrease in the mycobacterial burden in the spleens and livers of the animals (6, 8). In another study, however, an additive decrease in resistance as measured by an increase in mycobacterial CFU was observed in mice treated with a combination of antibodies to TNF- and gamma interferon (IFN-) compared to that observed after administration of either antibody alone (1). The addition of pentoxifylline, a chemical inhibitor of TNF-, to mice exhibit impaired phagocytic (13), NK (3, 29, 30), and T (2, 33)-cell functions, which constitute important mechanisms of immunoregulation and sources of TNF-. The current study also evaluated the power of C57BL/6 mice (5 to 6 weeks aged) were used in experiments which compared disease progression and serum TNF- production among the different strains of mice. All animals (Jackson Laboratories, Bar Harbor, Maine) were randomized and housed in groups of no more than five in microisolator cages and were fed ad libitum. Contamination of mice. MAC strain 101 (MAC 101) was cultured on Middlebrook 7H11 agar plates (Remel, Lenexa, Kan.). After 2 to 3 3 weeks of incubation, transparent colonies of MAC 101 were picked from your plates, suspended in sterile Middlebrook 7H9 broth (Difco Laboratories, c-Fms-IN-9 Detroit, Mich.), aliquoted, and frozen at ?70C as the stock culture (5 108 to 1 1 109 CFU/ml) for all those infection studies. The mice were infected intravenously with 5 to 6 107 CFU of MAC 101 in 7H9 broth. Control mice were sham infected with broth. Groups of five animals were sacrificed at weeks 1, 3, 5, and 8 following infection and evaluated for body weight, organ excess weight (spleen, liver, and lung), and microbial burden in the weighed subsections of these organs. Blood was collected for measurement of TNF- levels in the serum. A separate group of each strain of mice, infected (= 20) and uninfected (= 10), was set aside for a survival study. Microbial burden. Weighed sections of tissues (liver, lung, and spleen) were homogenized in Middlebrook 7H9 medium (Difco), and aliquots from different dilutions were plated onto Middlebrook 7H11 agar plates (Remel) in triplicate. c-Fms-IN-9 The cultures were incubated for 3 weeks at 37C in 7% CO2. TNF- levels. TNF- levels in the sera were measured by an enzyme-linked immunosorbent assay with kits obtained from Genzyme Diagnostics (Cambridge, Mass.). Treatment with TNF- inhibitors and measurement of disease progression. C57BL/6 value was found to be less than 0.05; therefore, no adjustment was imposed around the pairwise comparison of values. Differences in various parameters (including body weight, organ excess weight, microbial burden, and serum TNF- level) were determined by analysis of variance. Results of the microbial burden (in CFU) were analyzed after log transformation of the data. All values reported are the results of c-Fms-IN-9 two-tailed assessments, with no adjustment for multiple comparisons. RESULTS Susceptibility of C57BL/6 (and +/+ mice (week 5). However, by week 6, the mortality rates for mice. Mortality in mice continued to increase throughout the observation period, whereas the mortality rates stabilized at week 8 for both 0.05). The pairwise comparison showed the susceptibility of the strain (= 0.144). The +/+ mice were the least susceptible and were statistically different from the strain of mice c-Fms-IN-9 (= 0.014) but not from your = 0.373). Mycobacterial disease progression, as measured by increased organ weights (splenomegaly or hepatomegaly) and microbial burden, also developed in C57BL/6 mice at most time points. TABLE 1 Relative organ weights in three strains of C57BL/6 mice at 3 weeks following infection with MAC?101 0.05 compared to uninfected control.? Open in a separate windows FIG. 2 Microbial burden in three strains ( 0.05) compared to the controls.1991;146:3165C3170. has been associated with increased resistance to the infection, and inhibition of TNF- has been reported to decrease resistance. In vitro addition of TNF- to human or murine macrophages infected with resulted in increased intracellular killing of mycobacteria (4, 10, 19). Similarly, treatment of infected mice with TNF-, with or without interleukin 2 (IL-2), resulted in a decrease in the mycobacterial burden in the spleens and livers of the animals (6, 8). In another study, however, an additive decrease in resistance as measured by an increase in mycobacterial CFU was observed in mice treated with a combination of antibodies to TNF- and gamma interferon (IFN-) compared to that observed after administration of either antibody alone (1). The addition of pentoxifylline, a chemical inhibitor of TNF-, to mice exhibit impaired phagocytic (13), NK (3, 29, 30), and T (2, 33)-cell functions, which constitute important mechanisms of immunoregulation and sources of TNF-. The current study also evaluated the power of C57BL/6 mice (5 to 6 weeks aged) were used in experiments which compared disease progression and serum TNF- production among the different strains of mice. All animals (Jackson Laboratories, Bar Harbor, Maine) were randomized and housed in groups of no more than five in microisolator cages and were fed ad libitum. Contamination of mice. MAC strain 101 (MAC 101) was cultured on Middlebrook 7H11 agar plates (Remel, Lenexa, Kan.). After 2 to 3 3 weeks of incubation, transparent colonies of MAC 101 were picked from your plates, suspended in sterile Middlebrook 7H9 broth (Difco Laboratories, Detroit, Mich.), aliquoted, and frozen at ?70C as the stock culture (5 108 to 1 1 109 CFU/ml) for all those infection studies. The mice were infected intravenously with 5 to 6 107 CFU of MAC 101 in 7H9 broth. Control mice were sham infected with broth. Groups of five animals were sacrificed at weeks 1, 3, 5, and 8 following infection and evaluated for body weight, organ excess weight (spleen, liver, and lung), and microbial burden in the weighed subsections of these organs. Blood was collected for measurement of TNF- levels in the serum. A separate group of each strain of mice, infected (= 20) and uninfected (= 10), was set aside for a survival study. Microbial burden. Weighed sections of tissues (liver, lung, and spleen) were homogenized in Middlebrook 7H9 medium (Difco), and aliquots from different dilutions were plated onto Middlebrook 7H11 agar plates (Remel) in triplicate. The cultures were incubated for 3 weeks at 37C in 7% CO2. TNF- levels. TNF- levels in the sera were measured by an enzyme-linked immunosorbent assay with kits obtained from Genzyme Diagnostics (Cambridge, Mass.). Treatment with TNF- inhibitors and measurement of disease development. C57BL/6 worth was found to become significantly less than 0.05; consequently, no modification was imposed for the pairwise assessment of values. Variations in various guidelines (including bodyweight, organ pounds, microbial burden, and serum TNF- level) had been determined by evaluation of variance. Outcomes from the microbial burden (in CFU) had been examined after log change of the info. All ideals reported will be the outcomes of two-tailed testing, with no modification for multiple evaluations. Outcomes Susceptibility of C57BL/6 (and +/+ mice (week 5). Nevertheless, by week 6, the mortality prices for mice. Mortality in mice continuing to increase through the entire observation period, whereas the mortality prices stabilized at week 8 for both 0.05). The pairwise assessment demonstrated the susceptibility of any risk of strain (= 0.144). The +/+ mice had been the least vulnerable and had been statistically not the same as any risk of strain of mice (= 0.014) however, not through the = 0.373). Mycobacterial disease development, as assessed by improved body organ weights (splenomegaly or hepatomegaly) and microbial burden, also created in C57BL/6 mice for the most part period factors. TABLE 1 Comparative body organ weights in three strains of C57BL/6 mice at 3 weeks pursuing infection with Mac pc?101 0.05 in comparison to uninfected control.? Open up in another home window FIG. 2 ABH2 Microbial burden in three strains ( 0.05) set alongside the controls (naive and vehicle-treated organizations). The uninfected mice from both from the treated organizations did not display significant degrees of serum TNF- at the period points tested. Open up in another home window FIG. 5 Aftereffect of treatment with dexamethasone (10.
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